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Progress toward ultrafast DNA sequencing using solid-state nanopores.利用固态纳米孔实现超快速DNA测序的进展。
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Extracting kinetics from single-molecule force spectroscopy: nanopore unzipping of DNA hairpins.从单分子力谱学中提取动力学:DNA发夹的纳米孔解链
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The electromechanics of DNA in a synthetic nanopore.合成纳米孔中DNA的机电学
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Nanopore unzipping of individual DNA hairpin molecules.单个DNA发夹分子的纳米孔解链
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A nanosensor for transmembrane capture and identification of single nucleic Acid molecules.一种用于跨膜捕获和识别单个核酸分子的纳米传感器。
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Fabrication of solid-state nanopores with single-nanometre precision.具有单纳米精度的固态纳米孔的制造。
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使用合成的亚2纳米孔对单个DNA分子进行机电解链。

Electromechanical unzipping of individual DNA molecules using synthetic sub-2 nm pores.

作者信息

McNally Ben, Wanunu Meni, Meller Amit

机构信息

Department of Biomedical Engineering, Department of Physics, Boston University, Boston, Massachusetts, USA.

出版信息

Nano Lett. 2008 Oct;8(10):3418-22. doi: 10.1021/nl802218f. Epub 2008 Aug 30.

DOI:10.1021/nl802218f
PMID:18759490
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2906227/
Abstract

Nanopores have recently emerged as high-throughput tools for probing and manipulating nucleic acid secondary structure at the single-molecule level. While most studies to date have utilized protein pores embedded in lipid bilayers, solid-state nanopores offer many practical advantages which greatly expand the range of applications in life sciences and biotechnology. Using sub-2 nm solid-state nanopores, we show for the first time that the unzipping kinetics of individual DNA duplexes can be probed by analyzing the dwell-time distributions. We performed high-bandwidth electrical measurements of DNA duplex unzipping as a function of their length, sequence, and temperature. We find that our longer duplexes (>10 bp) follow Arrhenius dependence on temperature, suggesting that unzipping can be approximated as a single-barrier crossing, but the unzipping kinetics of shorter duplexes do not involve a barrier, due to the strong biasing electrical force. Finally, we show that mismatches in the duplex affect unzipping times in a position-sensitive manner. Our results are a crucial step toward sequence variability detection and our single-molecule nanopore sequencing technology, which rely on parallel detection from nanopore arrays.

摘要

纳米孔最近已成为在单分子水平探测和操纵核酸二级结构的高通量工具。虽然迄今为止的大多数研究都使用了嵌入脂质双层的蛋白质孔,但固态纳米孔具有许多实际优势,极大地扩展了其在生命科学和生物技术中的应用范围。使用亚2纳米固态纳米孔,我们首次表明,通过分析驻留时间分布可以探测单个DNA双链体的解链动力学。我们对DNA双链体解链进行了高带宽电学测量,测量结果是其长度、序列和温度的函数。我们发现,较长的双链体(>10个碱基对)的解链动力学符合阿累尼乌斯温度依赖关系,这表明解链可以近似为单个势垒穿越过程,但较短双链体的解链动力学不涉及势垒,这是由于强大的偏置电力所致。最后,我们表明双链体中的错配以位置敏感的方式影响解链时间。我们的研究结果是朝着序列变异检测以及我们的单分子纳米孔测序技术迈出的关键一步,该技术依赖于来自纳米孔阵列的并行检测。